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Infection and Immunity, September 2000, p. 5096-5106, Vol. 68, No. 9
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Construction and Phenotypic Evaluation of a
Vibrio vulnificus vvpE Mutant for Elastolytic
Protease
Kwang Cheol
Jeong,1
Hye Sook
Jeong,1
Joon Haeng
Rhee,2
Shee Eun
Lee,2
Sun Sik
Chung,2
Angela M.
Starks,3
Gloria M.
Escudero,3
Paul A.
Gulig,3 and
Sang Ho
Choi1,*
Department of Food Science and Technology,
Institute of Biotechnology, Chonnam National University, Kwang-Ju,
500-757,1 and Department of
Microbiology, Chonnam National University Medical School, Kwang-Ju,
500-190,2 South Korea, and Department of
Molecular Genetics and Microbiology, College of Medicine,
University of Florida, Gainesville, Florida
32610-02663
Received 25 April 2000/Accepted 6 June 2000
Vibrio vulnificus is an opportunistic gram-negative
pathogen that commonly contaminates oysters. Predisposed individuals
who consume raw oysters can die within days from sepsis, and even otherwise healthy people are susceptible to serious wound infection after contact with contaminated seafood or seawater. Numerous secreted
and cell-associated virulence factors have been proposed to account for
the fulminating and destructive nature of V. vulnificus infections. Among the putative virulence factors is an elastolytic metalloprotease. We cloned and sequenced the vvpE gene
encoding an elastase of V. vulnificus ATCC 29307. The
functions of the elastase were assessed by constructing
vvpE insertional knockout mutants and evaluating phenotypic
changes in vitro and in mice. Although other types of protease activity
were still observed in vvpE mutants, elastase activity was
completely absent in the mutants and was restored by reintroducing the
recombinant vvpE gene. In contrast to previous
characterization of elastase as a potential virulence factor, which was
demonstrated by injecting the purified protein into animals,
inactivation of the V. vulnificus vvpE gene did not affect
the ability of the bacteria to infect mice and cause damage, either
locally in subcutaneous tissues or systemically in the liver, in both
iron-treated and normal mice. Furthermore, a vvpE mutant
was not affected with regard to cytolytic activity toward INT407
epithelial cells or detachment of INT407 cells from culture dishes in
vitro. Therefore, it appears that elastase is less important in the
pathogenesis of V. vulnificus than would have been
predicted by examining the effects of administering purified proteins
to animals. However, V. vulnificus utilizes a variety of
virulence factors; hence, the effects of inactivation of elastase alone
could be masked by other compensatory virulence factors.
*
Corresponding author. Mailing address: Department of
Food Science and Technology, Institute of Biotechnology, Chonnam
National University, Kwang-Ju, 500-757, South Korea. Phone:
82-62-530-2146. Fax: 82-62-530-2149. E-mail:
shchoi{at}chonnam.chonnam.ac.kr.
Infection and Immunity, September 2000, p. 5096-5106, Vol. 68, No. 9
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
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